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US11241689B2 - Microchip electrophoresis inkjet dispensing - Google Patents

Microchip electrophoresis inkjet dispensingDownload PDF

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US11241689B2
US11241689B2US15/670,896US201715670896AUS11241689B2US 11241689 B2US11241689 B2US 11241689B2US 201715670896 AUS201715670896 AUS 201715670896AUS 11241689 B2US11241689 B2US 11241689B2
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exit channel
pump chamber
discharge outlet
electrophoresis
electrophoresis column
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Michael D. Furtaw
Donald T. Lamb
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Li Cor Biotech LLC
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Li Cor Inc
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Abstract

Devices and methods are provided for the separation and dispensing of material using a microfluidic electrophoresis column, sheath liquid pump, and exit channel, all on the same monolithic chip. Material is separated in the electrophoresis column and passed into the exit chamber in response to a voltage potential between a first electrode within the electrophoresis column and a terminating electrode integrated into the chip. The terminating electrode can be in the sheath liquid pump chamber, the sheath liquid reservoir, or a separate flow channel that intersects the exit channel along with the electrophoresis column and sheath liquid pump chamber. The flow of sheath liquid into the exit chamber entrains separated analytes into an effluent that is dispensed out of the exit chamber via a discharge outlet.

Description

CROSS-REFERENCES TO RELATED APPLICATIONS
The present application claims the benefit of U.S. Provisional Appln. No. 62/372,244 filed Aug. 8, 2016, the full disclosure which is incorporated herein by reference in its entirety for all purposes.
STATEMENT AS TO RIGHTS TO INVENTIONS MADE UNDER FEDERALLY SPONSORED RESEARCH AND DEVELOPMENT
This invention was made with government support under Grant No. 1R43GM112289-01 awarded by the National Institutes of Health. The government has certain rights in the invention.
BACKGROUND
Western blotting is a ubiquitous analytical technique for identifying and quantifying specific proteins in a complex mixture. In the technique, gel electrophoresis is used to separate proteins in a gel based on properties such as tertiary structure, molecular weight, isoelectric point, polypeptide length, or electrical charge. Once separated, the proteins are then transferred from the gel to a membrane—typically made of nitrocellulose, nylon, or polyvinylidene fluoride (PVDF)—that binds proteins non-specifically. A commonly used method for carrying out this transfer is electroblotting, in which an electrical current is used to pull proteins from the gel into the membrane. The membrane is then stained with probes specific for the proteins being targeted, allowing the location and amounts of these proteins to be detected.
Capillary electrophoresis provides an alternative to the gel electrophoresis separation associated with western blotting and other biotechnology procedures. In capillary electrophoresis, materials such as proteins are separated electrokinetically, as in gel electrophoresis, but with much smaller required volumes. The capillaries used in this technique are typified by diameters smaller than one millimeter and are in some instances incorporated into microfluidic or nanofluidic devices.
Previous work has demonstrated the benefits of applying microfluidic devices to Western blotting of proteins (Jin et al. 2013Anal. Chem.85:6073). These devices electrically transfer separated proteins to a blotting surface that is itself the terminating electrode. (See, e.g., U.S. Pat. No. 9,182,371). This electrical field blotting approach requires continuous electrical contact from a separation device to the surface. As a result, the surface must be electrically conductive (e.g., a wet membrane on metal platen).
In electric field blotting, proteins migrate toward the surface via electrophoresis. Since the cross-sectional area of the current flow abruptly increases upon exiting the separation device, the electric field abruptly diminishes. Also, since the surface is typically wet, a large meniscus tends to form around the point of contact between the separation device and the surface. This large meniscus can comprise recirculation zones in which analytes such as proteins can be trapped and mixed, reducing the resolution of separation. Furthermore, the electrical field blotting force is only applied while the separation device is above the analyte. If a surface and separation device move to a different position relative to one another, the electrical force is removed and only diffusion forces cause the analyte to become immobilized in the surface membrane.
Alternative dispensing techniques such as, for example, inkjetting of material, can address some of the above issues. Inkjet dispensing is a mature and well-understood technology that is often used in commercial printers (Martin et al. 2008J. Physics: Conference Series105:012001). Over the past several years, inkjet technology has been used in an increasing variety of applications where the dispensing of small, controllable amounts of fluid is required (Derby 2010Ann. Rev. Mat. Res.40:395).
BRIEF SUMMARY
In general, provided herein are devices and methods for the dispensing of small, controllable amounts of material that have been separated by microfluidic electrophoresis. The separated material outputs from an electrophoretic column into an exit channel. Bulk flow of a sheath fluid passes through the exit channel and entrains the analytes in an effluent that is discharged from the exit channel through an outlet. Each of the electrophoresis column, exit channel, and sheath flow pump are integrated on a single chip. The electrophoretic flow is driven by a voltage potential between two electrodes that are also integrated onto the chip. The terminating electrode can be located within a separate flow channel that is also connected to the exit channel such that material flows electrophoretically from the electrophoresis column towards the flow channel and into the exit channel. Multiple electrophoresis columns can be integrated onto the same chip. A terminating electrode within a single common flow channel can be used to generate multiple voltage potentials with multiple electrodes located within multiple electrophoresis columns.
One provided apparatus comprises an electrophoresis column having an input end and an output end, wherein the input end has an opening configured to accept a fluid sample. The apparatus further comprises a first electrode proximate to and in fluidic connection with the input end of the electrophoresis column. The apparatus further comprises a sheath liquid reservoir. The apparatus further comprises a pump chamber connected to the sheath liquid reservoir, wherein the pump comprises an impulsive pump element. The apparatus further comprises an exit channel having an upstream end and a downstream end. The upstream end is connected to the pump chamber and the downstream end has a discharge outlet. The output end of the electrophoresis column intersects the exit channel. The apparatus further comprises a second electrode in fluidic connection with the exit chamber.
In some embodiments, the second electrode is within the pump chamber. In some embodiments, the apparatus further comprises a flow channel, wherein the flow channel intersects the exit channel. In some embodiments, the second electrode is within or upstream of the flow channel. In some embodiments, the apparatus further comprises a sieving matrix, wherein the sieving matrix is inside the electrophoresis column.
In some embodiments, the impulsive pump element comprises a piezoelectric material configured to deform at least a portion of the pump chamber. The impulsive pump element comprises a thermoresistive element configured to form a bubble in a sheath liquid when the sheath liquid is within the pump chamber. In some embodiments, the impulsive pump element comprises an solenoid valve configured to alternatingly open and close. In some embodiments, In some embodiments, the electrophoresis column, pump chamber, and exit channel are integrated on a single monolithic chip.
In some embodiments, the apparatus further comprises a surface positioned across a gap from the discharge outlet. In some embodiments, the apparatus further comprises a motor configured to move the surface laterally with respect to the discharge outlet. In some embodiments, the apparatus further comprises a motor configured to move the discharge outlet laterally with respect to the surface. In some embodiments, the surface comprises a hydrophobic material. In some embodiments, the surface comprises a hydrophilic material. In some embodiments, the surface includes a blotting membrane. In some embodiments, the surface comprises a matrix-assisted laser desorption/ionization (MALDI) plate. In some embodiments, the surface comprises a microtiter plate.
Also provided is an apparatus comprising a first and second electrophoresis column. The first electrophoresis column has a first input end and a first output end, and the second electrophoresis column has a second input end and a second output end. The first input end has a first opening configured to accept a first fluid sample, and the second output end has a second opening configured to accept a second fluid sample. The apparatus further comprises a first and second electrode. The first electrode is proximate to and in fluidic connection with the first input end of the first electrophoresis column, and the second electrode is proximate to and in fluidic connection with the second input end of the second electrophoresis column. The apparatus further comprises a first and second sheath liquid reservoir. The apparatus further comprises a first and second pump chamber. The first pump chamber is connected to the first sheath liquid reservoir, and the second pump chamber is connected to the second sheath liquid reservoir. The apparatus further comprises a first and second impulsive pump element. The first impulsive pump element is configured to impulsively deform at least a portion of the first pump chamber, and the second impulsive pump element is configured to impulsively deform at least a portion of the second pump chamber. The apparatus further comprises a first and second exit channel. The first exit channel has a first upstream end and a first downstream end, and the second exit channel has a second upstream end and a second downstream end. The first upstream end is connected to the first pump chamber, and the second upstream end is connected to the second pump chamber. The first downstream end has a first discharge outlet, and the second downstream end has a second discharge outlet. The first output end of the first electrophoresis column intersects the first exit channel, and the second output end of the second electrophoresis column intersects the second exit channel. The apparatus further comprises a common flow channel, wherein the common flow channel intersects the first and second exit channels. The apparatus further comprises a third electrode within the common flow channel.
In some embodiments, the first and second electrophoresis columns, first and second pump chambers, common flow channel, and first and second exit channels are integrated on a single monolithic chip.
Also provided is a method of dispensing one or more analytes from an electrophoresis column. The method comprises applying a voltage potential between an input end of an electrophoresis column and an output end of the electrophoresis column, wherein the voltage potential continues outside of the output end and into an exit channel. The output end of the electrophoresis column intersects the exit channel. The exit channel has an upstream end and a downstream end. The upstream end of the exit channel is connected to a pump chamber, and the downstream end of the exit channel has a discharge outlet. The pump chamber is connected to a sheath liquid reservoir. The voltage is sufficient to electrophorese one or more analytes from the input end of the electrophoresis column to the output end of the electrophoresis column. The method further comprises impulsively deforming the pump chamber sufficiently to pump a sheath liquid from the sheath liquid reservoir to the exit channel. The method further comprises entraining the one or more analytes in the sheath liquid to form an effluent. The method further comprises dispensing the effluent through the discharge outlet of the exit channel.
In some embodiments, the voltage potential continues outside of the output end of the electrophoresis column, through a portion of the exit channel, and into the pump chamber. In some embodiments, the voltage potential continues outside of the output end of the electrophoresis column, through a portion of the exit channel, and into a flow channel, wherein the flow channel intersects the exit channel.
In some embodiments, the dispensing creates one or more droplets. In some embodiments, the dispensing creates a stream. In some embodiments, the method further comprises contacting the dispensed effluent with a surface. In some embodiments, the method further comprises moving the surface relative to the discharge outlet. In some embodiments, the method further comprises moving the discharge outlet relative to the surface. In some embodiments, the surface comprises a hydrophobic material. In some embodiments, the surface comprises a hydrophilic material. In some embodiments, the surface includes a blotting membrane. In some embodiments, the surface comprises a matrix-assisted laser desorption/ionization (MALDI) plate. In some embodiments, the surface comprises a microtiter plate.
Also provided is a method of dispensing two or more analytes from two electrophoresis columns. The method comprises applying a first voltage potential between a first input end of a first electrophoresis column and a common flow channel. A first output end of the first electrophoresis column intersects a first exit channel, and the common flow channel intersects the first exit channel. The first exit channel has a first upstream end and a first downstream end. The first upstream end of the first exit channel is connected to a first pump chamber, and the first downstream end of the first exit channel has a first discharge outlet. The first pump chamber is connected to a first sheath liquid reservoir. The first voltage is sufficient to electrophorese one or more of the two or more analytes from the first input end of the first electrophoresis column to the first output end of the first electrophoresis column. The method further comprises applying a second voltage potential between a second input end of a second electrophoresis column and the common flow channel. A second output end of the second electrophoresis column intersects a second exit channel, and the common flow channel intersects the second exit channel. The second exit channel has a second upstream end and a second downstream end. The second upstream end of the second exit channel is connected to a second pump chamber, and the second downstream end of the second exit channel has a second discharge outlet. The second pump chamber is connected to a second sheath liquid reservoir. The second voltage is sufficient to electrophorese one or more of the two or more analytes from the second input end of the second electrophoresis column to the second output end of the second electrophoresis column. The method further comprises impulsively deforming the first pump chamber sufficiently to pump a first sheath liquid from the first sheath liquid reservoir to the first exit channel. The method further comprises impulsively deforming the second pump chamber sufficiently to pump a second sheath liquid from the second sheath liquid reservoir to the second exit channel. The method further comprises entraining one or more of the two or more analytes in the first sheath liquid to form a first effluent, and entraining one or more of the two or more analytes in the second sheath liquid to form a second effluent. The method further comprises dispensing the first effluent through the first discharge outlet of the first exit channel, and dispensing the second effluent through the second discharge outlet of the second exit channel.
In some embodiments, each dispensing step creates one or more droplets. In some embodiments, each dispensing step creates a stream. In some embodiments, the method further comprises contacting the dispensed first and second effluents with a surface. In some embodiments, the method further comprises moving the surface relative to the first and second discharge outlets. In some embodiments, the method further comprises moving the first and second discharge outlets relative to the surface. In some embodiments, the surface comprises a hydrophobic material. In some embodiments, the surface comprises a hydrophilic material. In some embodiments, the surface includes a blotting membrane. In some embodiments, the surface comprises a matrix-assisted laser desorption/ionization (MALDI) plate. In some embodiments, the surface comprises a microtiter plate.
BRIEF DESCRIPTION OF THE DRAWINGS
FIG. 1 illustrates a microfluidic separation and dispensing device in accordance with an embodiment and having a terminating electrode upstream of a pump chamber.
FIG. 2 illustrates a microfluidic separation and dispensing device in accordance with an embodiment and having a terminating electrode within a flow channel.
FIG. 3 illustrates a microfluidic separation and dispensing device in accordance with an embodiment and having two electrophoresis columns and a terminating electrode within a common flow channel.
FIG. 4 illustrates an intersection between an electrophoresis column, a flow channel, and an exit channel, wherein the intersection is configured as a cross.
FIG. 5 illustrates an intersection between an electrophoresis column, a flow channel, and an exit channel, wherein the intersection is configured as an offset cross.
FIG. 6 is illustrates an intersection between an electrophoresis column and an exit channel.
FIG. 7 is a flowchart of a process for separating and dispensing an analyte from an electrophoresis column in accordance with an embodiment.
FIG. 8 is a flowchart of a process for separating and dispensing analytes from two electrophoresis columns in accordance with an embodiment.
DETAILED DESCRIPTION
Embodiments of the present invention relate to the dispensing of material output from one or more microfluidic separation columns. The material is dispensed by using inkjet technology to “jet” proteins or other separated analytes from the separation column and onto a surface. The use of the inkjet technology relieves any electrical requirements of the surface substrate.
The disclosed embodiments can be used to enable high-resolution blotting of molecules onto a solid support as they elute from a separation column. The blotting can be, for example, analogous to western blotting. The disclosed embodiments can work with a wide variety of dispensed droplet sizes (e.g., 10 pL-10 nL) and frequencies (e.g., 0-10,000 Hz). Biomolecules are not fragmented during the separation and dispensing processes. The separation column can be spatially isolated from the solid support with no need to maintain a liquid connection. Antibodies and/or blocking reagents can be dispensed with low volume consumption. This and other dispensing processes can be operated independently of any separation process. Blotting can be with the use of discrete drops to maintain separation resolution and enable novel detection strategies. Furthermore, hydrophobic surface substrates can be used to gain sensitivity by concentrating dispensed material to smaller dot sizes. Fraction collection operations are also enabled with the disclosed embodiments. These fraction collection operations using material separated with microfluidics can be as straightforward as common fraction collection operations typically used with material separated with larger-scale chromatography. The use of microfluidics can further enable faster separations, better resolution, the use of smaller sample amounts, the elimination of tubing connections and “dead volume” within the system, and the enabling of massive parallelization.
FIG. 1 illustrates a microfluidic separation and dispensing apparatus in accordance with an embodiment. Shown indevice100 is anelectrophoresis column101 having aninput end102 and anoutput end103. Theinput end102 has anopening104 configured to accept a fluid sample. Afirst electrode105 is proximate to and in fluid connection with theinput end102 of theelectrophoresis column101. Also shown is asheath liquid reservoir106, and apump chamber107 connected to the sheath liquid reservoir. Animpulsive pump element108 is configured to impulsively deform at least a portion of thepump chamber107. Also shown is anexit channel109 having anupstream end110 and adownstream end111. Theupstream end110 of theexit channel109 is connected to thepump chamber107. Thedownstream end111 of theexit channel109 has adischarge outlet112. Theoutput end103 of theelectrophoresis column101 intersects with theexit channel109. Asecond electrode113 is in fluidic connection with theexit chamber109.
The term “fluidic connection” as used herein refers to a connection between two or more enclosed or semi-enclosed volumes, such that a fluid within one of the volumes can flow to each of the other volumes. In this way, the volumes in fluidic connection with one another form a hydraulic circuit. It is to be understood that a fluid need not be present in any of the volumes for the volumes to be in fluidic connection with one another.
FIG. 2 illustrates another microfluidic separation and dispensing apparatus in accordance with an embodiment. Thedevice200 ofFIG. 2 is similar to that depicted inFIG. 1, further comprising aflow channel201 that intersects theexit channel202. Thesecond electrode203 ofdevice200 is within theflow channel201, and not within thepump chamber204 orsheath flow reservoir205, as is shown inFIG. 1. Theflow channel201 is on the same singlemonolithic chip207 as theelectrophoresis column206,pump chamber204, andexit channel202.
The electrophoresis column can be formed from, for example, plastic or fused silica. In some embodiments, the diameters of the input and output ends of the electrophoresis column are in a range from about 5 μm to about 500 μm. In some embodiments, the diameters of the input and output ends are about 1 μm, 5 μm, 10 μm, 20 μm, 30 μm, 40 μm, 50 μm, 60 μm, 70 μm, 80 μm, 90 μm, 100 μm, 110 μm, 120 μm, 130 μm, 140 μm, 150 μm, 160 μm, 170 μm, 180 μm, 190 μm, 200 μm, 210 μm, 220 μm, 230 μm, 240 μm, 250 μm, 260 μm, 270 μm, 280 μm, 290 μm, 300 μm, 310 μm, 320 μm, 330 μm, 340 μm, 350 μm, 360 μm, 370 μm, 380 μm, 390 μm, 400 μm, 410 μm, 420 μm, 430 μm, 440 μm, 450 μm, 460 μm, 470 μm, 480 μm, 490 μm, 500 μm, 600 μm, 700 μm, 800 μm, 900 μm, or 1000 μm. The diameters of the input and/or output ends can be, for example and without limitation, within the range between 1 μm and 60 μm, between 2 μm and 130 μm, between 4 μm and 250 μm, between 8 μm and 500 μm, or between 15 μm and 1000 μm. The diameters of the input and/or output ends can be within the range between 5 μm and 80 μm, between 8 μm and 125 μm, between 12 μm and 200 μm, between 20 μm and 325 μm, or between 30 μm and 500 μm.
The first and second electrodes can be formed from any conducting or semiconducting material. For example, one or both or the electrodes can comprise a metal. In some embodiments, the metal is gold or platinum. In some embodiments, one or both of the electrodes are platinum or can be platinum-plated. One or both of the electrodes can be substantially cylindrical in shape, as in a wire. One or both of the electrodes can be substantially flattened in shape so as to increase their surface area.
The sheath liquid reservoir can have a volume of less than 10 ml, less than 6.5 ml, less than 4 ml, less than 2.5 ml, less than 1.5 ml, less than 1 ml, less than 650 μl, less than 400 μl less than 250 μl, less than 150 μl, less than 100 μl, less than 65 μl, less than 40 μl, less than 25 μl, less than 15 μl, or less than 10 μl. The sheath liquid reservoir can, for example and without limitation, have a volume within the range between 10 μl and 650 μl, between 20 μl and 1.25 ml, between 40 μl and 2.5 ml, between 80 μl and 5 ml, or between 150 μl and 10 ml.
The pump chamber can be formed from, for example, plastic or fused silica. In some embodiments, the diameter of the pump chamber is in a range from about 5 μm to about 500 μm. In some embodiments, the diameter of the pump chamber is 1 μm, 5 μm, 10 μm, 20 μm, 30 μm, 40 μm, 50 μm, 60 μm, 70 μm, 80 μm, 90 μm, 100 μm, 110 μm, 120 μm, 130 μm, 140 μm, 150 μm, 160 μm, 170 μm, 180 μm, 190 μm, 200 μm, 210 μm, 220 μm, 230 μm, 240 μm, 250 μm, 260 μm, 270 μm, 280 μm, 290 μm, 300 μm, 310 μm, 320 μm, 330 μm, 340 μm, 350 μm, 360 μm, 370 μm, 380 μm, 390 μm, 400 μm, 410 μm, 420 μm, 430 μm, 440 μm, 450 μm, 460 μm, 470 μm, 480 μm, 490 μm, 500 μm, 600 μm, 700 μm, 800 μm, 900 μm, or 1000 μm. The diameter of the pump chamber can be, for example and without limitation, within the range between 1 μm and 60 μm, between 2 μm and 130 μm, between 4 μm and 250 μm, between 8 μm and 500 μm, or between 15 μm and 1000 μm. The diameter of the pump chamber can be within the range between 5 μm and 80 μm, between 8 μm and 125 μm, between 12 μm and 200 μm, between 20 μm and 325 μm, or between 30 μm and 500 μm.
The impulsive pump element can alter the physical properties of the pump chamber by transferring or converting energy into an acoustic wave. The impulsive pump element can alter the physical properties of the pump chamber by adjusting a mechanical stress on the pump chamber. The impulsive pump can be a thermal inkjet, wherein the impulsive pump element is a thermoresistive material. The impulsive pump can comprise a solenoid valve configured to rapidly open and close. The impulsive pump element can have a deformable surface. The deformable surface can be configured to expand, to contract, or both. The movement of the deformable surface alters the volume of the pump internal region. As the volume of the pump internal region decreases, the pressure of material within the pump internal region increases. In this way, the pump can affect pressure-driven flow of sheath liquid from the sheath liquid reservoir to the exit channel.
The impulsive pump can comprise a piezoelectric material. In some embodiments, the impulsive pump comprises a piezoelectric crystal. In some embodiments, the impulsive pump comprises lead zirconate titanate. The impulsive pump can comprise a thermoresistive material. The impulsive pump can be electrically connected to an impulsive pump actuator. In some embodiments, the impulsive pump actuator can transmit a signal to the impulsive pump causing it to expand.
The exit channel can have a substantially constant cross-sectional diameter along its length from the upstream end to the downstream end. The exit channel can be tapered such that the cross-sectional diameter of the exit channel proximate to the discharge outlet is smaller than the cross-sectional area of the exit channel proximate to the output end of the electrophoresis column. In some embodiments, the entire internal region of the exit channel is tapered. In some embodiments, only the portion of the exit region proximate to the discharge outlet is tapered. The tapering can be such that the cross-sectional area of the exit channel decreases linearly along the longitudinal axis of the exit channel. The tapering can be such that cross-sectional area of the exit channel decreases nonlinearly along the longitudinal axis of the exit channel. In a preferred embodiment, the exit channel substantially does not taper.
The discharge outlet can have any shape that is capable of allowing the formation of droplets of dispensed fluid. The discharge outlet can have a circular or ovoid shape. The discharge outlet can have a triangular, rectangular, or other polygonal shape. The discharge outlet shape can have two or more axes of symmetry. The discharge outlet can be symmetrical along three axis. The diameter or major axis of the discharge outlet can be larger than, equal to, or smaller than the diameter of the capillary outlet. In some embodiments, the diameter of the discharge outlet is within the range from about 5 μm to about 200 μm. The diameter of the discharge outlet can be in the range between about 5 μm and about 500 μm. The diameter of the discharge outlet can be, for example, in a range between about 5 μm and about 80 μm, between about 10 μm and about 125 μm, between about 15 μm and about 200 μm, between about 20 μm and about 300 μm, or between about 30 μm and about 500 μm. The diameter of the discharge outlet can be between about 20 μm and about 60 μm, between about 25 μm and about 70 μm, between about 30 μm and about 85 μm, between about 35 μm and about 100 μm, or between about 40 μm and about 125 μm. In some embodiments, the diameter of the discharge outlet is about 50 μm. In some embodiments, the diameter of the discharge outlet is about 1 μm, 5 μm, 10 μm, 20 μm, 30 μm, 40 μm, 50 μm, 60 μm, 70 μm, 80 μm, 90 μm, 100 μm, 110 μm, 120 μm, 130 μm, 140 μm, 150 μm, 160 μm, 170 μm, 180 μm, 190 μm, 200 μm, 210 μm, 220 μm, 230 μm, 240 μm, 250 μm, 260 μm, 270 μm, 280 μm, 290 μm, 300 μm, 310 μm, 320 μm, 330 μm, 340 μm, 350 μm, 360 μm, 370 μm, 380 μm, 390 μm, 400 μm, 410 μm, 420 μm, 430 μm, 440 μm, 450 μm, 460 μm, 470 μm, 480 μm, 490 μm, 500 μm, 600 μm, 700 μm, 800 μm, 900 μm, or 1000 μm.
In a preferred embodiment, the discharge outlet is located along a centerline of the exit channel. Alternatively, the discharge outlet can offset from the centerline of the exit channel. Preferably, at least a portion of the exit channel proximate to the discharge outlet has a substantially smooth surface. As used herein, the term “substantially smooth” refers to a surface that is completely or mostly free of texturing such as voids, protrusions, grooves, or ridges. A surface can have minor indentations or raised portions, or other imperfections not intended during manufacture, and still be considered to be substantially smooth. The smoothness of the exit channel and discharge outlet can depend at least in part on aspects of the manufacturing process (e.g., polishing, dicing, scribing, or lasering), and can influence the morphology of droplets dispensed from the device.
Theelectrophoresis column206,pump chamber204, andexit channel202 ofdevice200 ofFIG. 2 can all be located on a singlemonolithic chip207. The chip can comprise, for example, one or more of silicon, glass, polydimethylsiloxane (PDMS), polymethylmethacrylate (PMMA), cyclic olefin polymer (COP), cyclic olefin copolymer (COC) or quartz.
Also shown inFIG. 2 is asurface208 that is positioned across agap209 from thedischarge outlet210. In some embodiments, the surface comprises an electrically insulating material. In some embodiments, the surface comprises an electrically conductive material. In some embodiments, the surface comprises a hydrophilic material. In some embodiments, the surface comprises a hydrophobic material. In some embodiments, the surface comprises a matrix-assisted laser desorption/ionization (MALDI) plate. For example, the surface can be a metal plate configured to receive spotting of a solution containing MALDI samples. In some embodiments, the surface comprises a microtiter plate. For example, the surface can be the inner surface of a well of a microtiter plate, or can be an array of 6, 24, 96, 384, 1536, or other number of wells forming a microtiter plate.
In some embodiments, the surface is wet. In some embodiments, the surface is dry. The use of a dry surface can be advantageous for multiple reasons. One advantage of a dry surface is the elimination of any operating complexities associated with the maintaining of a consistently wet membrane. Another advantage is that a dry membrane can provides a capillary, or “wicking”, force as an effluent exits the discharge outlet. As discussed below, this can assist with immobilization of proteins or other analytes.
In some embodiments, the discharge outlet contacts the surface. In some embodiments, the surface is positioned across a gap from the discharge outlet and the discharge outlet does not contact the surface. Because the terminating electrode is located on the chip of the device, there is not an electrical requirement for the surface, and the surface and an effluent exiting from the discharge outlet do not require continuous electrical contact. The surface can be a dry membrane, plastic, glass, etc. In some embodiments, the surface is located about 0.1 mm, 0.2 mm, 0.3 mm, 0.4 mm, 0.5 mm, 0.6 mm, 0.7 mm, 0.8 mm, 0.9 mm, 1 mm, 2 mm, 3 mm, 4 mm, 5 mm, 6 mm, 7 mm, 8 mm, 9 mm, 10 mm, 20 mm, 30 mm, 40 mm, 50 mm, 60 mm, 70 mm, 80 mm, 90 mm, or 100 mm from the discharge outlet. The gap between the surface and the discharge outlet can be, for example and without limitation, within the range between 0.1 mm and 6 mm, between 0.2 mm and 12 mm, between 0.4 mm and 25 mm, between 0.8 mm and 50 mm, or between 2 mm and 100 mm.
In some embodiments, the surface is a component of a fraction collection device. In some embodiments, the surface is located within a well of a microtiter plate. The microtiter plate can comprise an array of a plurality of wells. The number of wells arrayed on the microtiter plate can be, for example, 6, 24, 96, 384, 1536, 3456, or 9600, or more.
Also shown inFIG. 2 is amotor211 configured to move one or both of thesurface208 or thechip207. The motor can be configured to move the surface laterally with respect to the discharge outlet. The motor can be configured to move the discharge outlet laterally with respect to the surface. The motor can be, for example, a stepper motor, small brushed direct current (DC) motor, or brushless DC motor. The motor can be an element of a robotic apparatus that is programmed or otherwise configured to automate and/or regulate the operation of the motor. Movement can be continuous or semi-continuous. Movement can stop intermittently for sample or fraction collection.
Because the terminating electrode is located within a flow channel of the device, the discharge outlet and/or surface can be moved away from one another without interrupting the separation process. This can increase the throughput of separation and dispensing by allowing other electrical processes, such as those associated with separations or sample injections, to continue while the discharge outlet and/or surface are moved relative to one another. This also enables fraction collection operations in which an effluent stream or series of droplets is first collected in one well before the device is repositioned above an adjacent well while the separation processes continue.
Also shown inFIG. 2 is ablotting membrane212 that is an optional element of thesurface208. In some embodiments, the surface is a blotting membrane that can be useful for performing a western immunoassay or other membrane analysis methods such as northern blotting and Southern blotting. The method can further comprise applying a detection reagent to such a blotting membrane. The detection reagent can be an antibody such as a primary or secondary antibody.
The term “antibody” includes a polypeptide encoded by an immunoglobulin gene or functional fragments thereof that specifically binds and recognizes an antigen. Immunoglobulin genes include the kappa, lambda, alpha, gamma, delta, epsilon, and mu constant region genes, as well as the myriad immunoglobulin variable region genes. Light chains are classified as either kappa or lambda. Heavy chains are classified as gamma, mu, alpha, delta, or epsilon, which in turn define the immunoglobulin classes, IgG, IgM, IgA, IgD and IgE, respectively. The term antibody activity, or antibody function, refers to specific binding of the antibody to the antibody target.
A primary antibody will be understood by one of skill to refer to an antibody or fragment thereof that specifically binds to an analyte (e.g., substance, antigen, component) of interest. The primary antibody can further comprise a tag, e.g., for recognition by a secondary antibody or associated binding protein (e.g., green fluorescent protein, biotin, or strepavidin).
A secondary antibody refers to an antibody that specifically binds to a primary antibody. A secondary antibody can be specific for the primary antibody (e.g., specific for primary antibodies derived from a particular species) or a tag on the primary antibody (e.g., GFP, biotin, or strepavidin). A secondary antibody can be bispecific, e.g., with one variable region specific for a primary antibody, and a second variable region specific for a bridge antigen.
Blotting membranes can comprise, for example, nitrocellulose, nylon, polyvinylidene difluoride, or combinations of one or more of these materials. The blotting membrane can further comprise a support material. The support material can be, for example, glass, plastic, metal, ceramic or other inert surface.
In some embodiments, a region of the membrane immediately across from the discharge outlet is dry until wetted by an effluent exiting from the discharge outlet. The effluent can be in the form of, for example, a continuous stream, a semi-continuous stream, or discrete droplets. In some embodiments, the degree of hydrophobicity of the surface affects the surface area of droplets once contacted with the surface. In general, for aqueous droplets, as the hydrophobicity of the surface increases, the contact angle of the droplets with the surface will decrease. This decreased contact angle can allow the distances between adjacent droplets on the surface to be reduced while still preventing droplets from coalescing or otherwise combining with one another. In this way, the use of a hydrophobic surface material can enable a greater concentration of distinct droplets to be dispensed onto the surface. Also, for each individual droplet, the concentration of dispensed material per unit of area of the contacted surface material will increase. In some embodiments, this increased concentration can lead to greater signal intensities for applications such as western blotting.
In some embodiments, the surface material is selected such that adjacent droplets dispensed onto the surface remain distinct. These embodiments can generate dispensed patterns that maintain the resolution of the separation of material within the separation column and the dispensing apparatus. In some embodiments, the surface material is selected such that adjacent droplets dispensed onto the surface coalesce. Through movement of one or both of the surface and/or the dispensing apparatus during dispensing, these embodiments can generate dispensed patterns that are continuous linear or curved representations of the separation of material within the electrophoresis column.
The effluent can comprise an analyte. In some embodiments, the effluent is wicked into the membrane. In some embodiments, the analyte becomes immobilized in the membrane upon wicking of the effluent into the membrane. In some embodiments, the effluent is pulled toward the dry membrane until the substrate is saturated. Therefore, for embodiments in which the surface and/or discharge outlet move relative to one another, the immobilization force may continue in membrane surface locations that are no longer directly beneath the discharge outlet. At relatively low sheath flow rates (typically <1 μl/min) the meniscus between the discharge outlet and the membrane can be narrow and recirculation zones can be minimal.
Any of the devices described above can be used to separate one or more analytes moving within the separation column. An “analyte” includes a substance of interest such as a biomolecule. Biomolecules are molecules of a type typically found in a biological system, whether such molecule is naturally occurring or the result of some external disturbance of the system (e.g., a disease, poisoning, genetic manipulation, etc.), as well as synthetic analogs and derivatives thereof. Non-limiting examples of biomolecules include amino acids (naturally occurring or synthetic), peptides, polypeptides, glycosylated and unglycosylated proteins (e.g., polyclonal and monoclonal antibodies, receptors, interferons, enzymes, etc.), nucleosides, nucleotides, oligonucleotides (e.g., DNA, RNA, PNA oligos), polynucleotides (e.g., DNA, cDNA, RNA, etc.), carbohydrates, hormones, haptens, steroids, toxins, etc. Biomolecules can be isolated from natural sources, or they can be synthetic.
The analytes can be, for example, proteins, nucleic acids, carbohydrates, lipids, or any other type of molecule. In some embodiments, the analytes are proteins that are present in the separation column in their native state. In some embodiments, the analytes are proteins that have been mixed with sodium dodecyl sulfate to cause their partial or complete denaturation.
Also shown inFIG. 2 is a sievingmatrix213 inside theelectrophoresis column206. Protein and DNA size-based separation techniques often rely on gels or polymer solutions to resolve populations of biomolecules. These gels and polymer solutions create a random sieving media through which the biomolecules migrate, separating the molecules by size as they pass through the media. The composition and porosity of conventional separation media can be modified to produce pores of different average sizes within the media.
The sieving matrix can contain a substantially heterogeneous or substantially homogeneous assortment of pore sizes. The sieving matrix can comprise nanoparticles, beads, macromolecules, a colloidal crystal, a gel, a polymer solution, or other medium. The sieving matrix can comprise silica nanoparticles that form a colloidal crystal, providing a separation media which has a substantially monodisperse pore size, based on the monodispersity of the silica colloid size and the crystallization of the colloids. The use of separation media comprising silica nanoparticles is further discussed in U.S. Patent Application Publication No. 2015/0279648A1, as published Oct. 1, 2015, which is entirely incorporated by reference herein for all purposes.
The sieving matrix can comprise, for example, one or more of sodium dodecyl sulfate (SDS), polyvinylpyrrolidone (PVP), polyethylene oxide (PEO), polylactic acid (PLA), polyethylene glycol (PEG), polydimethylacrylamide (PDMA), acrylamide, polyacrylamide, methylcellulose, hydroxypropylmethyl cellulose (HPMC), hydroxypropyl cellulose (HPC), hydroxyethyl cellulose (HEC), agarose gel, or dextran.
Also provided are devices that comprise a plurality of individual dispensing units. The dispensing units can be configured in a linear array. The dispensing units can be configured in a 2-dimensional array. In some embodiments, the device comprises 1, 2, 4, 8, 12, or more dispensing units. The dispensing units can each be connected to the same supply of sheath liquid. The dispensing units can each be connected to different supplies of sheath liquid.
FIG. 3 illustrates another microfluidic separation and dispensing apparatus in accordance with an embodiment. Shown indevice300 are a first301 and second302 electrophoresis column. Thefirst electrophoresis column301 has afirst input end303 and afirst output end304, and thesecond electrophoresis column302 has a second input end305 and asecond output end306. Thefirst input end303 has afirst opening307 configured to accept a first sample, and the second input end305 has asecond opening308 configured to accept a second sample.
Also shown inFIG. 3 are a first309 and second310 electrode. The first electrode309 is proximate to and in fluidic connection with thefirst input end303 of thefirst electrophoresis column301, and the second electrode310 is proximate to and in fluidic connection with the second input end305 of thesecond electrophoresis column302. Also shown are a first311 and second312 sheath liquid reservoir. Afirst pump chamber313 is connected to the firstsheath liquid reservoir311, and asecond pump chamber314 is connected to the secondsheath liquid reservoir312. A firstimpulsive pump element315 is configured to impulsively deform at least a portion of thefirst pump chamber313, and a secondimpulsive pump chamber316 is configured to impulsively deform at least a portion of thesecond pump chamber314.
Also shown inFIG. 3 are a first317 and second318 exit channel. The first exit channel317 has a firstupstream end319 and a firstdownstream end320, and thesecond exit channel318 has a secondupstream end321 and a seconddownstream end322. The firstupstream end319 is connected to thefirst pump chamber313, and the secondupstream end321 is connected to thesecond pump chamber314. The firstdownstream end320 has afirst discharge outlet323, and the seconddownstream end322 has asecond discharge outlet324. Thefirst output end304 of thefirst electrophoresis column301 intersects the first exit channel317, and thesecond output end306 of thesecond electrophoresis column302 intersects thesecond exit channel318. Also shown is acommon flow channel325 that intersects both the first317 and second318 exit channels. Athird electrode326 is within thecommon flow channel325. In some embodiments, and as is shown inFIG. 3, each of the first301 and second302 electrophoresis columns, the first313 and second314 pump chambers, the first317 and second318 exit channels, and thecommon flow channel325 are integrated on a singlemonolithic chip327.
The common flow channel can be formed from, for example, plastic or fused silica. In some embodiments, the diameter of the common flow channel is in a range from about 5 μm to about 500 μm. In some embodiments, the diameter of the common flow channel is about 1 μm, 5 μm, 10 μm, 20 μm, 30 μm, 40 μm, 50 μm, 60 μm, 70 μm, 80 μm, 90 μm, 100 μm, 110 μm, 120 μm, 130 μm, 140 μm, 150 μm, 160 μm, 170 μm, 180 μm, 190 μm, 200 μm, 210 μm, 220 μm, 230 μm, 240 μm, 250 μm, 260 μm, 270 μm, 280 μm, 290 μm, 300 μm, 310 μm, 320 μm, 330 μm, 340 μm, 350 μm, 360 μm, 370 μm, 380 μm, 390 μm, 400 μm, 410 μm, 420 μm, 430 μm, 440 μm, 450 μm, 460 μm, 470 μm, 480 μm, 490 μm, 500 μm, 600 μm, 700 μm, 800 μm, 900 μm, or 1000 μm. The diameter of the common flow channel can be, for example and without limitation, within the range between 1 μm and 60 μm, between 2 μm and 130 μm, between 4 μm and 250 μm, between 8 μm and 500 μm, or between 15 μm and 1000 μm. The diameter of the common flow channel can be within the range between 5 μm and 80 μm, between 8 μm and 125 μm, between 12 μm and 200 μm, between 20 μm and 325 μm, or between 30 μm and 500 μm.
The third electrode can be formed from any conducting or semiconducting material. For example, the third electrode can comprise a metal. In some embodiments, the metal is gold or platinum. In some embodiments, the third electrode is platinum or can be platinum-plated. The third electrode can be substantially cylindrical in shape, as in a wire. The third electrode can be substantially flattened in shape so as to increase their surface area.
Although the above description is of a device using two columns to dispense two or more analytes, it is appreciated that a similar device can comprise three or more columns to dispense three or more analytes. For example, a device can comprise three, four, five, six, seven, eight, nine, ten, or more than ten columns. Such devices can further comprise multiple sheath liquid reservoirs, pump chambers, and exit channels, each configured to be in fluidic connection with one of the multiple columns. Such devices can further comprise multiple common channels, each configured to connect with adjacent pairs of exit channels on the device.
FIG. 4 illustrates an intersection between anelectrophoresis column401, aflow channel402, and anexit channel403, wherein the intersection is configured as a cross. A voltage potential between a first electrode404 located within theelectrophoresis column401 and asecond electrode405 located within theflow channel402 can driveelectrophoretic flow406 of separatedanalytes407 through theelectrophoresis column401 and into theexit channel403. Apump408 generatesbulk flow409 through theexit channel403 and out adischarge outlet410. Thebulk flow409 sweepsanalyte407 passing through the intersection out of thedischarge outlet410 in the form of aneffluent droplet411.
FIG. 5 illustrates a different intersection between anelectrophoresis column501, aflow channel502, and anexit channel503, wherein the intersection is configured as an offset cross. With the configuration shown inFIG. 5, the electrophoretic flow504 of separatedanalytes505 causes the analytes to travel further upstream in theexit channel503 relative to the direction of bulk flow506 as compared to the configuration shown inFIG. 4. This can increase the residence time ofanalytes505 within theexit channel503. As a result,more analyte505 can be swept out of the discharge outlet507 in each effluent droplet508 while the pump509 is configured to produce droplets at a lower frequency than with the device configuration shown inFIG. 4.
FIG. 6 illustrates a different intersection between anelectrophoresis column601 and anexit channel602. A voltage potential between a first electrode603 located within theelectrophoresis column601 and asecond electrode604 located within theexit channel602 can drive electrophoretic flow605 of separatedanalytes606 through theelectrophoresis column601 and into theexit channel602. With the configuration shown inFIG. 6, the analytes can travel further upstream in theexit channel602 relative to the direction ofbulk flow607 as compared to the configurations shown inFIGS. 4 and 5. This can further increase the residence time ofanalytes606 within theexit channel602. Thepump608 can be configured to periodically clear theexit channel602 by producing one or moreeffluent droplets609 to sweep accumulatedanalytes606 out of through thedischarge outlet610. In this way, the device can operate somewhat similarly to a traditional fraction collector, but with much higher separation and resolution capabilities.
FIG. 7 presents a flowchart of aprocess700 for dispensing one or more analytes from an electrophoresis column. Inoperation701, a voltage potential is applied between an input end of an electrophoresis column and an output end of the electrophoresis column. The voltage potential continues outside of the output end and into an exit channel. The output end of the electrophoresis column intersects the exit channel, wherein the exit channel has an upstream end and a downstream end. The upstream end of the exit channel is connected to a pump chamber, and the downstream end of the exit channel has a discharge outlet. The pump chamber is connected to a sheath liquid reservoir. The voltage is sufficient to electrophorese one or more analytes from the input end of the electrophoresis column to the output end of the electrophoresis column. Inoperation702, the pump chamber is impulsively deformed sufficiently to pump a sheath liquid from the sheath liquid reservoir to the exit channel. In operation703, the one or more analytes are entrained in the sheath liquid to form an effluent. Inoperation704, the effluent is dispensed through the discharge outlet of the exit channel.
The voltage at the first electrode is held at a different voltage than that at the second electrode. The difference in voltages causes analytes in the separation column to separate from one another in a technique known as electrophoresis. Electrophoresis is the induced motion of particles suspended in a fluid by an electric field, or as otherwise known in the art. Electrophoresis of positively charged particles (cations) is often called cataphoresis, while electrophoresis of negatively charged particles (anions) is often called anaphoresis.
The power for applying a voltage can supply an electric field having voltages of about 1 V/cm to 2000 V/cm. In some embodiments, the voltage is about 1 V/cm, 10 V/cm, 20 V/cm, 30 V/cm, 40 V/cm, 50 V/cm, 60 V/cm, 70 V/cm, 80 V/cm, 90 V/cm, 100 V/cm, 150 V/cm, 200 V/cm, 250 V/cm, 300 V/cm, 350 V/cm, 400 V/cm, 450 V/cm, 500 V/cm, 550 V/cm, 600 V/cm, 650 V/cm, 700 V/cm, 750 V/cm, 800 V/cm, 850 V/cm, 900 V/cm, 950 V/cm, 1000 V/cm, 1050 V/cm, 1100 V/cm, 1150 V/cm, 1200 V/cm, 1250 V/cm, 1300 V/cm, 1350 V/cm, 1400 V/cm, 1450 V/cm, 1500 V/cm, 1550 V/cm, 1600 V/cm, 1650 V/cm, 1700 V/cm, 1750 V/cm, 1800 V/cm, 1850 V/cm, 1900 V/cm, 1950 V/cm, or 2000 V/cm. The voltage can be, for example and without limitation, within the range between 1 V/cm and 100 V/cm, between 2 V/cm and 200 V/cm, between 5 V/cm and 400 V/cm, between 10 V/cm and 900 V/cm, or between 20 V/cm and 2000 V/cm. Higher voltages can also be used, depending on the particular separation method.
Motion of analytes or other material within the separation column can occur solely through electrophoresis. There can also be a bulk fluid flow through the separation column that contributes to the motion of analytes or other material. In some embodiments, the analytes or other materials within the separation column move only through the action of bulk fluid flow within the tube.
In certain aspects, the electrophoresis systems and methods of the present invention resolve or separate the analyte as a function of the pI of the analyte. The isoelectric point (pI) is the pH at which a particular molecule carries no net electrical charge. Other suitable techniques for resolution or separation include, but are not limited to, electrophoresis, isoelectric focusing, isotachophoresis, ion exchange chromatography, cation exchange chromatography, and hydrophobic interaction chromatography. Resolution can also be conducted using affinity chromatography, wherein separation results from interaction of one or more analytes with binding moieties such as antibodies, lectins, and aptamers, in the separation bed.
In some embodiments, one or more analytes are separated within the the separation column by isoelectric focusing prior to subsequent movement of the analytes within the column by a bulk fluid flow. In some embodiments, one or more analytes are moved within the separation column by a bulk fluid flow prior to their subsequent separation within the column by isoelectric focusing. In one provided embodiment of a method, an isoelectric focusing step is used to separate one or more analytes within the column, a bulk fluid flowing step is used to move the one or more analytes into the dispensing apparatus, and a dispensing step is used to dispense the one or more analytes onto a surface.
The movement of material within the exit channel is determined in part by the presence, directions, and magnitudes of sheath liquid flows, bulk fluid flow output from the separation column, and an electrical field within the separation column and the exit channel. In some embodiments, the contribution of bulk fluid flow is greater than that of an electrical field, and accordingly the movement of material within the exit channel is in a direction substantially towards the discharge outlet.
In some embodiments, the method further comprises controlling the pressure of the sheath liquid in the sheath liquid reservoir that is in fluidic connection with the pump chamber. In some embodiments, the method further comprises controlling the pressure of an electrophoresis solution in an electrophoresis solution reservoir that is in fluidic connection with the electrophoresis column.
The liquid that exits the microfluidic discharge outlet can consist entirely of sheath liquid. The liquid that exits the microfluidic nozzle can consist entirely of material that is output from the capillary electrophoresis tube. In some embodiments, the liquid that exits the microfluidic nozzle comprises a mixture of sheath liquid and material that is output from the capillary electrophoresis tube, wherein the percentage of the mixture that comprises sheath liquid is about 0%, about 5%, about 10%, about 15%, about 20%, about 25%, about 30%, about 35%, about 40%, about 45%, about 50%, about 55%, about 60%, about 65%, about 70%, about 75%, about 80%, about 85%, about 90%, about 95%, or about 100%. The percentage of sheath fluid in the effluent liquid can be, for example and without limitation, within the range between 0% and 60%, between 10% and 70%, between 20% and 80%, between 30% and 90%, or between 40% and 100%.
In some embodiments, the voltage potential continues outside of the output end of the electrophoresis column, through a portion of the exit channel, and into the pump chamber. In some embodiments, the voltage potential continues outside of the output end of the electrophoresis column, through a portion of the exit channel, and into a flow channel, wherein the flow channel intersects the exit channel.
The dispensing can generate the formation of a continuous or discontinuous stream exiting the discharge outlet. The dispensing can generate the formation of droplets exiting the discharge outlet. The droplets can have volumes in the range from about 10 picoliter to about 10 nanoliter. The frequency of the droplets can be in a range from 0 to about 10,000 Hz.
The term “droplet” refers to a small volume of liquid, typically with a spherical shape, encapsulated by an immiscible fluid, such as a continuous phase or carrier liquid of an emulsion. In some embodiments, the volume of a droplet and/or the average volume of droplets is, for example, less than about one microliter (or between about one microliter and one nanoliter or between about one microliter and one picoliter), less than about one nanoliter (or between about one nanoliter and one picoliter), or less than about one picoliter (or between about one picoliter and one femtoliter), among others. In some embodiments, a droplet has a diameter (or an average diameter) of less than about 1000, 100, or 10 micrometers, or of about 1000 to 10 micrometers, among others. A droplet can be spherical or nonspherical. A droplet can be a simple droplet or a compound droplet, that is, a droplet in which at least one droplet encapsulates at least one other droplet.
The droplets can be monodisperse, that is, of at least generally uniform size, or can be polydisperse, that is, of various sizes. If monodisperse, the droplets can, for example, vary in volume by a standard deviation that is less than about plus or minus 100%, 50%, 20%, 10%, 5%, 2%, or 1% of the average droplet volume.
In some embodiments, the method further comprises contacting the dispensed effluent with a surface. In some embodiments, the method further comprises moving the surface relative to the discharge outlet. In some embodiments, the method further comprises moving the discharge outlet relative to the surface. The surface can be a hydrophobic material or a hydrophilic material. In some embodiments, the surface includes a blotting membrane.
FIG. 8 presents a flowchart of aprocess800 for dispensing two or more analytes from two electrophoresis columns. In operation801 a first voltage potential is applied between a first input end of a first electrophoresis column and a common flow channel. A first output end of the first electrophoresis column intersects a first exit channel, and the common flow channel intersects the first exit channel. The first exit channel has a first upstream end and a first downstream end. The first upstream end of the first exit channel is connected to a first pump chamber, and the first downstream end of the first exit channel has a first discharge outlet. The first pump chamber is connected to a first sheath liquid reservoir. The first voltage is sufficient to electrophorese one or more of the two or more analytes from the first input end of the first electrophoresis column to the first output end of the first electrophoresis column.
Inoperation802, a second voltage potential is applied between a second input end of a second electrophoresis column and the common flow channel. A second output end of the second electrophoresis column intersects a second exit channel, and the common flow channel intersects the second exit channel. The second exit channel has a second upstream end and a second downstream end. The second upstream end of the second exit channel is connected to a second pump chamber, and the second downstream end of the second exit channel has a second discharge outlet. The second pump chamber is connected to a second sheath liquid reservoir. The second voltage is sufficient to electrophorese one or more of the two or more analytes from the second input end of the second electrophoresis column to the second output end of the second electrophoresis column.
Inoperation803, the first pump chamber is impulsively deformed sufficiently to pump a first sheath liquid from the first sheath liquid reservoir to the first exit channel. Inoperation804, the second pump chamber is impulsively deformed sufficiently to pump a second sheath liquid from the second sheath liquid reservoir to the second exit channel. Inoperation805, one or more of the two or more analytes are entrained in the first sheath liquid to form a first effluent. Inoperation806, one or more of the two or more analytes are entrained in the second sheath liquid to form a second effluent. Inoperation807, the first effluent is dispensed through the first discharge outlet of the first exit channel. Inoperation808, the second effluent is dispensed through the second discharge outlet of the second exit channel.
The provided methods can further comprise moving the position of the surface relative to that of the dispensing device. The moving can comprise changing the location of the surface as the dispensing device is stationary. The moving can comprise changing the location of the dispensing device and the surface is stationary. The moving can comprise changing the locations of both the surface and the dispensing device. The moving can comprise changing the location of the surface in one direction and changing the location of the dispensing device in an orthogonal direction.
The number of electrophoresis columns and discharge outlets on a single chip can each independently be 2 or more, 3, or more, 4 or more, 5 or more, 6 or more, 7 or more, 8 or more, 9 or more, 10 or more, 15 or more, 20 or more, 25 or more, 30 or more, 35 or more, 40 or more, 45 or more, 50 or more, 60 or more, 70 or more, 80 or more, 90 or more, or 100 or more. In some embodiments, the number of electrophoresis columns and discharge outlets on a single chip is 10 or more. In some embodiments, the number of common flow channels on a single chip is n−1, where n is the number of electrophoresis columns on the chip.
Each reservoir of the apparatus can independently be connected to an off-chip reservoir. The volume of the off-chip reservoir can be at least 2-fold, 3-fold, 4-fold, 5-fold, 6-fold, 7-fold, 8-fold, 9-fold, 10-fold, 20-fold, 30-fold, 40-fold, 50-fold, 60-fold, 70-fold, 80-fold, 90-fold, 100-fold, 200-fold, 300-fold, 400-fold, 500-fold, 600-fold, 700-fold, 800-fold, 900-fold, or 1000-fold larger than that of the on-chip reservoir. In some embodiments, an electrode can be located within an off-chip reservoir. Electrical continuity between the off-chip reservoir and the on-chip elements of the apparatus can be through connecting tubing or channels. Two or more reservoirs of the apparatus can each be connected to a common off-chip reservoir. A reservoir of the apparatus can be connected to two or more off-chip reservoirs. A reservoir of the apparatus can be connected to two or more off-chip reservoirs through a selection valve, The selection valve can be configured to connect a selected off-chip reservoir to the on-chip reservoir depending on a selected method step. For example, different off-chip reservoirs can be connected for steps associated with conditioning, cleaning, waste disposal, sample injection, sample separation, or sample dispensing.
The method can utilize a computing apparatus that is programmed or otherwise configured to automate and/or regulate one or more steps of the method provided herein. Some embodiments provide machine executable code in a non-transitory storage medium that, when executed by a computing apparatus, implements any of the methods described herein. In some embodiments, the computing apparatus operates one or more of the pressure of reservoirs, the flow of liquid through columns and channels, the activity of an impulsive pump actuator, the moving of the surface, or the moving of the dispensing apparatus.
The term “automated” refers to a device, action, or method carried out by a machine or computer without direct human control. In some embodiments, the device and method described herein is operated in an automated fashion. In some embodiments, the automated method has subjective start and end points, thus the term does not imply that all steps of the operation are carried out automatically.
Systems that incorporate the apparatus are also provided. Systems can include, for example, a power supply and power regulator to control the current and/or voltage to the first and second electrodes and the impulsive pump actuator. Additionally, pumps and/or pressure sources for regulating the flow of liquids, mechanisms for stirring or mixing liquids, and heating or cooling units can be included.
It is understood that all devices and methods described above can further comprise flow channels, pumps, and reservoirs in addition to the ones described. In some embodiments, each flow channel, pump, and reservoir on one side of the separation column is mirrored by a similar flow channel, pump and reservoir on the opposite side of the separation column. In this way, the device can have a substantially or approximately symmetrical configuration. In some embodiments, the device has an asymmetrical configuration.
Reference to a “first” component does not necessarily require that a second component be provided. Moreover reference to a “first”, “second”, or “third” component does not limit the referenced component to a particular location unless expressly stated. The terms “first”, “second”, and “third” when used herein with reference to elements or properties are simply to more clearly distinguish the two or more elements or properties and unless stated otherwise are not intended to indicate order.
The terms “about” and “approximately equal” are used herein to modify a numerical value and indicate a defined range around that value. If “X” is the value, “about X” or “approximately equal to X” generally indicates a value from 0.90X to 1.10X. Any reference to “about X” indicates at least the values X, 0.90X, 0.91X, 0.92X, 0.93X, 0.94X, 0.95X, 0.96X, 0.97X, 0.98X, 0.99X, 1.01X, 1.02X, 1.03X, 1.04X, 1.05X, 1.06X, 1.07X, 1.08X, 1.09X, and 1.10X. Thus, “about X” is intended to disclose, e.g., “0.98X.” When “about” is applied to the beginning of a numerical range, it applies to both ends of the range. Thus, “from about 6 to 8.5” is equivalent to “from about 6 to about 8.5.” When “about” is applied to the first value of a set of values, it applies to all values in that set. Thus, “about 7, 9, or 11%” is equivalent to “about 7%, about 9%, or about 11%.”
It is understood that the examples and embodiments described herein are for illustrative purposes only and that various modifications or changes in light thereof will be suggested to persons skilled in the art and are to be included within the spirit and purview of this application and scope of the appended claims. All publications, patents, and patent applications, websites, and databases cited herein are hereby incorporated by reference in their entireties for all purposes.

Claims (20)

What is claimed is:
1. A microchip electrophoresis dispensing apparatus comprising:
an electrophoresis column having an input end and an output end, wherein the input end has an opening configured to accept a fluid sample;
a first electrode proximate to and in fluidic connection with the input end;
a terminating electrode in fluidic connection with the output end;
a sheath liquid reservoir;
a pump chamber connected to the sheath liquid reservoir;
an impulsive pump element configured to deform at least a portion of the pump chamber;
an exit channel having an upstream end connected to the pump chamber and a downstream end having a discharge outlet, wherein the output end of the electrophoresis column intersects the exit channel;
a surface positioned across a gap from the discharge outlet; and
a motor configured to move the surface or discharge outlet laterally with respect to one another,
wherein the surface is not electrically held at a voltage with respect to the first electrode or terminating electrode, and
wherein the impulsive pump element is configured to pump a sheath liquid from the sheath liquid reservoir to entrain analyte from the electrophoresis column and dispense the entrained analyte, as discrete droplets or a liquid stream, from the discharge outlet onto the surface.
2. The apparatus ofclaim 1 wherein the terminating electrode is within or upstream of the pump chamber.
3. The apparatus ofclaim 1 further comprising:
a flow channel, wherein the flow channel intersects the exit channel, and wherein the terminating electrode is within the flow channel.
4. The apparatus ofclaim 1 wherein the electrophoresis column, pump chamber, and exit channel are integrated on a single monolithic chip.
5. The apparatus ofclaim 1 wherein the surface supports a blotting membrane.
6. The apparatus ofclaim 1 further comprising:
a sieving matrix, wherein the sieving matrix is inside the electrophoresis column.
7. A method of dispensing one or more analytes from an electrophoresis column, the method comprising:
applying a voltage potential between an input end of an electrophoresis column and an output end of the electrophoresis column, wherein the voltage potential continues outside of the output end and into an exit channel, wherein the output end of the electrophoresis column intersects the exit channel, wherein the exit channel has an upstream end connect to a pump chamber and a downstream end having a discharge outlet, wherein the pump chamber is connected to a sheath liquid reservoir, and wherein the voltage is sufficient to electrophorese one or more analytes from the input end of the electrophoresis column to the output end of the electrophoresis column;
impulsively deforming the pump chamber, thereby pumping a sheath liquid from the sheath liquid reservoir to the exit channel;
entraining the one or more analytes in the sheath liquid to form an effluent;
dispensing the effluent through the discharge outlet of the exit channel;
contacting the dispensed effluent with a surface, positioned across a gap from the discharge outlet, wherein the surface is not held at a voltage with respect to the exit channel; and
moving the surface or discharge outlet relative to one another using a motor.
8. The method ofclaim 7 wherein the voltage potential continues outside of the output end of the electrophoresis column, through a portion of the exit channel, and into the pump chamber.
9. The method ofclaim 7 wherein the voltage potential continues outside of the output end of the electrophoresis column, through a portion of the exit channel, and into a flow channel, wherein the flow channel intersects the exit channel.
10. The method ofclaim 7 wherein the dispensing creates one or more droplets.
11. The method ofclaim 7 wherein the dispensing creates a liquid stream.
12. The method ofclaim 7 wherein the surface supports a blotting membrane.
13. The method ofclaim 10, wherein the average volume of the one or more droplets is less than about one nanoliter.
14. A microchip electrophoresis dispensing apparatus comprising:
an electrophoresis column having an input end and an output end, wherein the input end has an opening configured to accept a fluid sample;
a first electrode proximate to and in fluidic connection with the input end;
a terminating electrode in fluidic connection with the output end;
a sheath liquid reservoir;
a pump chamber connected to the sheath liquid reservoir;
an impulsive pump element configured to deform at least a portion of the pump chamber;
an exit channel having an upstream end connected to the pump chamber and a downstream end having a discharge outlet, wherein the output end of the electrophoresis column intersects the exit channel;
a flat surface positioned across a gap from the discharge outlet, wherein the flat surface is positioned between 6 mm and 100 mm from the discharge outlet; and
a motor configured to move the surface or discharge outlet laterally with respect to one another,
wherein the impulsive pump element is configured to pump a sheath liquid from the sheath liquid reservoir to entrain analyte from the electrophoresis column and dispense the entrained analyte, as discrete droplets or a liquid stream, from the discharge outlet onto the flat surface.
15. The apparatus ofclaim 14 wherein the terminating electrode is within or upstream of the pump chamber.
16. The apparatus ofclaim 14 further comprising:
a flow channel, wherein the flow channel intersects the exit channel, and wherein the terminating electrode is within the flow channel.
17. The apparatus ofclaim 14 wherein the electrophoresis column, pump chamber, and exit channel are integrated on a single monolithic chip.
18. The apparatus ofclaim 1, wherein the deforming of the pump chamber generates an acoustic wave.
19. The method ofclaim 7, wherein the deforming of the pump chamber generates an acoustic wave.
20. The apparatus ofclaim 14, wherein the deforming of the pump chamber generates an acoustic wave.
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Families Citing this family (10)

* Cited by examiner, † Cited by third party
Publication numberPriority datePublication dateAssigneeTitle
WO2016010748A1 (en)2014-07-142016-01-21Li-Cor, Inc.Analyte separator with electrohydrodynamic taylor cone jet blotter
CA3006200A1 (en)2015-11-302017-06-08Intabio, Inc.Devices and methods for sample characterization
WO2017136284A1 (en)2016-02-012017-08-10Li-Cor, Inc.Capillary electrophoresis inkjet dispensing
US10737268B2 (en)2016-08-082020-08-11Li-Cor, Inc.Multi-sheath flow and on-chip terminating electrode for microfluidic direct-blotting
CN109564188A (en)2016-08-082019-04-02利康公司 Microchip Electrophoretic Inkjet Dispensing
US10574426B2 (en)*2017-08-282020-02-25Avago Technologies International Sales Pte. LimitedFull duplex ranging systems and methods
CN111971112A (en)2018-01-292020-11-20因塔生物公司Devices, methods and kits for sample characterization
EP3811397B1 (en)2018-05-312024-09-18Intabio, LlcMethods for interfacing microfluidic systems with mass spectrometry
US11559944B2 (en)*2019-05-132023-01-24Drexel UniversityHigh resolution electrohydrodynamic three-dimensional printing of high viscosity materials
US11285484B2 (en)2019-08-122022-03-29Intabio, LlcMultichannel isoelectric focusing devices and high voltage power supplies

Citations (58)

* Cited by examiner, † Cited by third party
Publication numberPriority datePublication dateAssigneeTitle
US4631120A (en)1980-06-161986-12-23Fritz PohlMethod in which elemental particles electrophoretically migrate through a gel onto a collecting surface of a moving belt
US4885076A (en)1987-04-061989-12-05Battelle Memorial InstituteCombined electrophoresis-electrospray interface and method
US5094594A (en)*1990-04-231992-03-10Genomyx, IncorporatedPiezoelectric pumping device
US5234559A (en)1991-12-311993-08-10E. I. Du Pont De Nemours And CompanyApparatus for direct blotting and automated electrophoresis, transfer and detection and processes utilizing the apparatus thereof
US5275710A (en)1990-05-141994-01-04Labintelligence, Inc.Gel electrophoresis system including optical stage, sample applicator and sample retriever
US5393975A (en)1990-08-301995-02-28Finnigan CorporationElectrospray ion source and interface apparatus and method
US5423964A (en)1993-08-021995-06-13Battelle Memorial InstituteCombined electrophoresis-electrospray interface and method
US5474663A (en)1993-08-271995-12-12E. I. Du Pont De Nemours And CompanyBowed framed membrane, processes for the preparation thereof, and uses therefor
US5868322A (en)1996-01-311999-02-09Hewlett-Packard CompanyApparatus for forming liquid droplets having a mechanically fixed inner microtube
US5917184A (en)1996-02-081999-06-29Perseptive BiosystemsInterface between liquid flow and mass spectrometer
US5916429A (en)1997-08-011999-06-29Qualicon Inc.Direct blot electrophoresis apparatus and method
US6179584B1 (en)1996-12-112001-01-30Gesim Gesellschaft Fur Silizium-Mikrosysteme MbhMicroejector pump
US20010055529A1 (en)2000-06-092001-12-27Achim WixforthDevice and process for matter transport of small quantities of matter
US20020197622A1 (en)2001-01-312002-12-26Mcdevitt John T.Method and apparatus for the confinement of materials in a micromachined chemical sensor array
US6602391B2 (en)2001-03-052003-08-05Vladimir B. SerikovApparatus and method for combined capillary separation and blotting of biological macromolecules
US20030178563A1 (en)*2002-03-212003-09-25Thermo Finnigan LlcIonization apparatus and method for mass spectrometer system
US6633031B1 (en)1999-03-022003-10-14Advion Biosciences, Inc.Integrated monolithic microfabricated dispensing nozzle and liquid chromatography-electrospray system and method
US20030215855A1 (en)2002-04-022003-11-20Caliper Technologies Corp.Methods, systems and apparatus for separation and isolation of one or more sample components of a sample biological material
US20040058423A1 (en)2002-05-032004-03-25Nancy AlbrittonFast electrical lysis of cells and rapid collection of the contents thereof using capillary electrophoresis
US20040113068A1 (en)2001-09-192004-06-17Biospect Inc.Multi-channel microfluidic chip for electrospray ionization
US6787313B2 (en)1997-06-202004-09-07New York UniversityElectrospray apparatus for mass fabrication of chips and libraries
US20040247450A1 (en)2001-10-022004-12-09Jonatan KutchinskySieve electrooosmotic flow pump
US6830934B1 (en)1999-06-152004-12-14Lifescan, Inc.Microdroplet dispensing for a medical diagnostic device
US20040265182A1 (en)*2003-06-242004-12-30Chien-Hua ChenFluidic MEMS device
US20050023141A1 (en)2003-05-092005-02-03Amshey Joseph W.Solution phase electrophoresis device, components, and methods
US20050040328A1 (en)*2003-08-212005-02-24Applera CorporationReduction of matrix interference for MALDI mass spectrometry analysis
JP3775305B2 (en)2002-01-312006-05-17コニカミノルタホールディングス株式会社 Liquid mixing mechanism and liquid mixing method
US20060192107A1 (en)*2004-10-072006-08-31Devoe Donald LMethods and apparatus for porous membrane electrospray and multiplexed coupling of microfluidic systems with mass spectrometry
US20070035587A1 (en)2005-08-122007-02-15Jeong-Gun LeeDevices for printing biomolecular droplet on substrate and for printing ink on substrate or print paper using electric charge concentration effect and method of printing biomolecular droplet on substrate
US20070039866A1 (en)2005-08-222007-02-22Schroeder Benjamin GDevice, system, and method for depositing processed immiscible-fluid-discrete-volumes
US20090060797A1 (en)*2002-12-302009-03-05The Regents Of The University Of CaliforniaFluid control structures in microfluidic devices
CN101581728A (en)2008-05-132009-11-18索尼株式会社Microchip and channel structure for the same
CN101609088A (en)2008-06-162009-12-23索尼株式会社Flow sending method in micro-fluidic chip and the micro-fluidic chip
CN101613660A (en)2002-12-302009-12-30加州大学评议会 Methods and devices for detection and analysis of pathogens
US7759639B2 (en)2005-02-182010-07-20University Of South FloridaElectrospray depositing system for biological materials
US7784911B2 (en)2006-05-122010-08-31Samsung Electronics Co., Ltd.Apparatus and method for printing biomolecular droplet on substrate
US20110005932A1 (en)*2009-06-052011-01-13Integenx Inc.Universal sample preparation system and use in an integrated analysis system
US8293337B2 (en)2008-06-232012-10-23Cornell UniversityMultiplexed electrospray deposition method
US8294119B2 (en)2003-11-122012-10-23Universite Des Sciences Et Technologies De LillePlanar electronebulization sources modeled on a calligraphy pen and the production thereof
US20130032031A1 (en)2010-04-192013-02-07Battelle Memorial InstituteElectrohydrodynamic spraying
US20130140180A1 (en)2011-06-032013-06-06University Of Washington Through Its Center For CommercializationSheath-flow electrospray interface
US8470570B2 (en)2006-04-132013-06-25Samsung Electronics Co., Ltd.Apparatus and method for printing biomolecular droplet on substrate
US20130213811A1 (en)*2010-02-262013-08-22The Regents Of The University Of MichiganMicroscale western blot
US20130327936A1 (en)2011-03-112013-12-12The University Of North Carolina At Chapel HillMicrochips with integrated multiple electrospray ionization emitters and related methods, systems and devices
US20130337502A1 (en)*2012-06-082013-12-19Bruker Daltonik GmbhAnalysis of microbes from microcolonies by maldi mass spectrometry
US8613845B2 (en)2008-03-072013-12-24The University Of British ColumbiaSelf contained capillary electrophoresis system for interfacing with mass spectrometry
US20140014747A1 (en)2012-07-162014-01-16Bruker Daltonics, Inc.Assembly for an electrospray ion source
US20140319335A1 (en)*2011-11-222014-10-30Micromass Uk LimitedLow Cross-Talk Fast Sample Delivery System Based Upon Acoustic Droplet Ejection
WO2015019159A1 (en)2013-08-072015-02-12Dh Technologies Development Pte. Ltd.Bubble removal from liquid flow into a mass spectrometer source
WO2015031820A1 (en)2013-08-292015-03-05University Of Notre Dame Du LacHigh sensitivity electrospray interface
US20150247187A1 (en)2014-03-032015-09-03Biotec Umwelt-Analytik-Beratung-Service GmbhUse of pcr analysis for airborne nucleic acids
US20150279648A1 (en)2014-03-262015-10-01Li-Cor, Inc.Laser desorption ionization mass spectrometry using a particulate separation bed
US20160011149A1 (en)2014-07-142016-01-14Li-Cor, Inc.Analyte separator with electrohydrodynamic taylor cone jet blotter
US20160153944A1 (en)*2014-12-022016-06-02Micromass Uk LimitedRing Shaped Counter Electrode to Improve Beam Stability and Compound Sensitivity on a Ceramic Tile Type Microfluidic Device
US20170176386A1 (en)*2015-11-302017-06-22IntabioDevices and methods for sample characterization
US20170219522A1 (en)2016-02-012017-08-03Li-Cor, Inc.Capillary Electrophoresis Inkjet Dispensing
US20180036730A1 (en)2016-08-082018-02-08Li-Cor, Inc.Multi-Sheath Flow and On-Chip Terminating Electrode for Microfluidic Direct-Blotting
WO2018031483A1 (en)2016-08-082018-02-15Li-Cor, Inc.Microchip electrophoresis inkjet dispensing

Family Cites Families (2)

* Cited by examiner, † Cited by third party
Publication numberPriority datePublication dateAssigneeTitle
WO2010078601A1 (en)*2009-01-052010-07-08The Regents Of The University Of CaliforniaHigh throughput biomolecule separation and analysis
WO2014014529A2 (en)*2012-04-112014-01-23Brown UniversityRed, green, and blue lasing enabled by single-exciton gain colloidal quantum dot films

Patent Citations (65)

* Cited by examiner, † Cited by third party
Publication numberPriority datePublication dateAssigneeTitle
US4631120A (en)1980-06-161986-12-23Fritz PohlMethod in which elemental particles electrophoretically migrate through a gel onto a collecting surface of a moving belt
US4885076A (en)1987-04-061989-12-05Battelle Memorial InstituteCombined electrophoresis-electrospray interface and method
US5094594A (en)*1990-04-231992-03-10Genomyx, IncorporatedPiezoelectric pumping device
US5275710A (en)1990-05-141994-01-04Labintelligence, Inc.Gel electrophoresis system including optical stage, sample applicator and sample retriever
US5393975A (en)1990-08-301995-02-28Finnigan CorporationElectrospray ion source and interface apparatus and method
US5234559A (en)1991-12-311993-08-10E. I. Du Pont De Nemours And CompanyApparatus for direct blotting and automated electrophoresis, transfer and detection and processes utilizing the apparatus thereof
US5423964A (en)1993-08-021995-06-13Battelle Memorial InstituteCombined electrophoresis-electrospray interface and method
US5474663A (en)1993-08-271995-12-12E. I. Du Pont De Nemours And CompanyBowed framed membrane, processes for the preparation thereof, and uses therefor
US5868322A (en)1996-01-311999-02-09Hewlett-Packard CompanyApparatus for forming liquid droplets having a mechanically fixed inner microtube
US5917184A (en)1996-02-081999-06-29Perseptive BiosystemsInterface between liquid flow and mass spectrometer
US6179584B1 (en)1996-12-112001-01-30Gesim Gesellschaft Fur Silizium-Mikrosysteme MbhMicroejector pump
US6787313B2 (en)1997-06-202004-09-07New York UniversityElectrospray apparatus for mass fabrication of chips and libraries
US5916429A (en)1997-08-011999-06-29Qualicon Inc.Direct blot electrophoresis apparatus and method
US6633031B1 (en)1999-03-022003-10-14Advion Biosciences, Inc.Integrated monolithic microfabricated dispensing nozzle and liquid chromatography-electrospray system and method
US6830934B1 (en)1999-06-152004-12-14Lifescan, Inc.Microdroplet dispensing for a medical diagnostic device
US20010055529A1 (en)2000-06-092001-12-27Achim WixforthDevice and process for matter transport of small quantities of matter
US20020197622A1 (en)2001-01-312002-12-26Mcdevitt John T.Method and apparatus for the confinement of materials in a micromachined chemical sensor array
US6602391B2 (en)2001-03-052003-08-05Vladimir B. SerikovApparatus and method for combined capillary separation and blotting of biological macromolecules
US20040113068A1 (en)2001-09-192004-06-17Biospect Inc.Multi-channel microfluidic chip for electrospray ionization
US20040247450A1 (en)2001-10-022004-12-09Jonatan KutchinskySieve electrooosmotic flow pump
JP3775305B2 (en)2002-01-312006-05-17コニカミノルタホールディングス株式会社 Liquid mixing mechanism and liquid mixing method
US20030178563A1 (en)*2002-03-212003-09-25Thermo Finnigan LlcIonization apparatus and method for mass spectrometer system
US20030215855A1 (en)2002-04-022003-11-20Caliper Technologies Corp.Methods, systems and apparatus for separation and isolation of one or more sample components of a sample biological material
US20040058423A1 (en)2002-05-032004-03-25Nancy AlbrittonFast electrical lysis of cells and rapid collection of the contents thereof using capillary electrophoresis
CN101613660A (en)2002-12-302009-12-30加州大学评议会 Methods and devices for detection and analysis of pathogens
US20090060797A1 (en)*2002-12-302009-03-05The Regents Of The University Of CaliforniaFluid control structures in microfluidic devices
US20050023141A1 (en)2003-05-092005-02-03Amshey Joseph W.Solution phase electrophoresis device, components, and methods
US20040265182A1 (en)*2003-06-242004-12-30Chien-Hua ChenFluidic MEMS device
US20050040328A1 (en)*2003-08-212005-02-24Applera CorporationReduction of matrix interference for MALDI mass spectrometry analysis
US8294119B2 (en)2003-11-122012-10-23Universite Des Sciences Et Technologies De LillePlanar electronebulization sources modeled on a calligraphy pen and the production thereof
US20060192107A1 (en)*2004-10-072006-08-31Devoe Donald LMethods and apparatus for porous membrane electrospray and multiplexed coupling of microfluidic systems with mass spectrometry
US7759639B2 (en)2005-02-182010-07-20University Of South FloridaElectrospray depositing system for biological materials
US20070035587A1 (en)2005-08-122007-02-15Jeong-Gun LeeDevices for printing biomolecular droplet on substrate and for printing ink on substrate or print paper using electric charge concentration effect and method of printing biomolecular droplet on substrate
US20070039866A1 (en)2005-08-222007-02-22Schroeder Benjamin GDevice, system, and method for depositing processed immiscible-fluid-discrete-volumes
US8470570B2 (en)2006-04-132013-06-25Samsung Electronics Co., Ltd.Apparatus and method for printing biomolecular droplet on substrate
US7784911B2 (en)2006-05-122010-08-31Samsung Electronics Co., Ltd.Apparatus and method for printing biomolecular droplet on substrate
US8613845B2 (en)2008-03-072013-12-24The University Of British ColumbiaSelf contained capillary electrophoresis system for interfacing with mass spectrometry
CN101581728A (en)2008-05-132009-11-18索尼株式会社Microchip and channel structure for the same
CN101609088A (en)2008-06-162009-12-23索尼株式会社Flow sending method in micro-fluidic chip and the micro-fluidic chip
US8293337B2 (en)2008-06-232012-10-23Cornell UniversityMultiplexed electrospray deposition method
US20110005932A1 (en)*2009-06-052011-01-13Integenx Inc.Universal sample preparation system and use in an integrated analysis system
US9182371B2 (en)2010-02-262015-11-10The Regents Of The University Of MichiganMicroscale western blot
US20130213811A1 (en)*2010-02-262013-08-22The Regents Of The University Of MichiganMicroscale western blot
US20130032031A1 (en)2010-04-192013-02-07Battelle Memorial InstituteElectrohydrodynamic spraying
US20130327936A1 (en)2011-03-112013-12-12The University Of North Carolina At Chapel HillMicrochips with integrated multiple electrospray ionization emitters and related methods, systems and devices
US20130140180A1 (en)2011-06-032013-06-06University Of Washington Through Its Center For CommercializationSheath-flow electrospray interface
US20140319335A1 (en)*2011-11-222014-10-30Micromass Uk LimitedLow Cross-Talk Fast Sample Delivery System Based Upon Acoustic Droplet Ejection
US20130337502A1 (en)*2012-06-082013-12-19Bruker Daltonik GmbhAnalysis of microbes from microcolonies by maldi mass spectrometry
US20140014747A1 (en)2012-07-162014-01-16Bruker Daltonics, Inc.Assembly for an electrospray ion source
WO2015019159A1 (en)2013-08-072015-02-12Dh Technologies Development Pte. Ltd.Bubble removal from liquid flow into a mass spectrometer source
US20160181078A1 (en)2013-08-072016-06-23Dh Technologies Development Pte. Ltd.Bubble Removal from Liquid Flow into a Mass Spectrometer Source
US20150233877A1 (en)2013-08-292015-08-20University Of Notre Dame Du LacHigh sensitivity electrospray interface
WO2015031820A1 (en)2013-08-292015-03-05University Of Notre Dame Du LacHigh sensitivity electrospray interface
US9465014B2 (en)2013-08-292016-10-11University Of Notre Dame Du LacHigh sensitivity electrospray interface
US20150247187A1 (en)2014-03-032015-09-03Biotec Umwelt-Analytik-Beratung-Service GmbhUse of pcr analysis for airborne nucleic acids
US20150279648A1 (en)2014-03-262015-10-01Li-Cor, Inc.Laser desorption ionization mass spectrometry using a particulate separation bed
WO2016010748A1 (en)2014-07-142016-01-21Li-Cor, Inc.Analyte separator with electrohydrodynamic taylor cone jet blotter
US20160011149A1 (en)2014-07-142016-01-14Li-Cor, Inc.Analyte separator with electrohydrodynamic taylor cone jet blotter
US20160153944A1 (en)*2014-12-022016-06-02Micromass Uk LimitedRing Shaped Counter Electrode to Improve Beam Stability and Compound Sensitivity on a Ceramic Tile Type Microfluidic Device
US20170176386A1 (en)*2015-11-302017-06-22IntabioDevices and methods for sample characterization
US20170219522A1 (en)2016-02-012017-08-03Li-Cor, Inc.Capillary Electrophoresis Inkjet Dispensing
WO2017136284A1 (en)2016-02-012017-08-10Li-Cor, Inc.Capillary electrophoresis inkjet dispensing
US20180036730A1 (en)2016-08-082018-02-08Li-Cor, Inc.Multi-Sheath Flow and On-Chip Terminating Electrode for Microfluidic Direct-Blotting
WO2018031479A1 (en)2016-08-082018-02-15Li-Cor, Inc.Multi-sheath flow and on-chip terminating electrode for microfluidic direct-blotting
WO2018031483A1 (en)2016-08-082018-02-15Li-Cor, Inc.Microchip electrophoresis inkjet dispensing

Non-Patent Citations (44)

* Cited by examiner, † Cited by third party
Title
Amantonico et al., "Facile analysis of metabolites by capillary electrophoresis coupled to matrix-assisted laser desorption/ionization mass spectrometry using target plates with polysilazane nanocoating and grooves", Analyst, vol. 134, 2009, pp. 1536-1540.
Anderson et al., "Western Blotting using Capillary Electrophoresis", Analytical Chemistry, 2011, 1350-1355.
Application No. CN201780047883.3, Office Action, dated Jan. 6, 2021, 12 pages.
Application No. CN201780047902.2, Office Action, dated Jan. 6, 2021, 9 pages.
AU2017213725, First Examination Report, dated May 7, 2021, 2 pages.
Avseenko et al., "Immobilization of Proteins in Immunochemical Microarrays Fabricated by Electrospray Deposition", Anal. Chem. vol. 73, 2001, pp. 6047-6052.
Avseenko et al., "Immunoassay with Multicomponent Protein Microarrays Fabricated by Electrospray Deposition", Anal. Chem., vol. 74, 2002, pp. 927-933.
Back et al., "Capillary Electrophoresis with Nanoparticle Matrix for DNA Analysis", Bull. Korean Chem. Soc., vol. 27, No. 1, 2006, pp. 133-136.
Delaney et al., "Inkjet printing of proteins", Soft Matter, vol. 5, 2009, pp. 4866-4877.
Derby , "Inkjet Printing of Functional and Structural Materials: Fluid Property Requirements, Feature Stability, and Resolution", Annu. Rev. Mater. Res. 40, 2010, pp. 395-414.
Ertl et al., "Capillary Electrophoresis Chips with a Sheath-Flow Supported Electrochemical Detection System", Analytical Chemistry, vol. 76, No. 13, Jul. 1, 2004, pp. 3749-3755.
European Application No. EP17747982.1, "Extended European Search Report," dated Aug. 7, 2019, 10 pages.
Gast et al., "The development of integrated microfluidic systems at GeSiM", Lab on a Chip, 3, 2003, pp. 6N-10N.
Han et al., "BioPen: direct writing of functional material at the point of care", Scientific Reports vol. 4, Article No. 4872, 2014, pp. 1-5.
Helmja et al., "Fraction collection in capillary electrophoresis for various stand-alone mass spectrometers", Journal of Chromatography A, vol. 1216, 2009, pp. 3666-3673.
Hou et al., "Direct detection and drug-resistance profiling of bacteremias using inertial microfluidics", Lab on a Chip, vol. 15, No. 10, 2015, pp. 2297-2307.
International Search Report and written opinion for PCT/US2015/039121 dated Sep. 30, 2015, 9 pages.
International Search Report and Written Opinion for PCT/US2017/015657 dated Apr. 4, 2017, 18 pages.
International Search Report dated Dec. 22, 2017 for corresponding PCT Appln. No. PCT/US2017/045778, 5 pages.
Jaworek et al., "Electrospraying route to nanotechnology: An overview", Journal of Electrostatics, vol. 66, 2008, pp. 197-219.
Jin et al., "Western Blotting Using Microchip Electrophoresis Interfaced to a Protein Capture Membrane", Analytical Chemistry 85(12), 2013, 6073-6079.
Johnson et al., "A CE-MALDI Interface Based on the Use of Prestructured Sample Supports", Anal. Chem.,vol. 73, 2001, pp. 1670-1675.
Kim et al., "Design and evaluation of single nozzle with a non-conductive tip for reducing applied voltage and pattern width in electrohydrodynamic jet printing (EHDP)", J. Micromech. Microeng, vol. 20, 2010, pp. 7.
Korkut et al., "Enhanced Stability of Electrohydrodynamic Jets through Gas Ionization", PRL,vol. 100, 2008, pp. 034503-1-034503-4.
Lu et al., "Coupling Sodium Dodecyl Sulfate-Capillary Polyacrylamide Gel Eletrophoresis with Matrix-Assisted Laser Desorption Ionization Time-of-Flight Mass Spectrometry via a Poly(tetrafluoroethylene) Membrane", Anal. Chem., vol. 83, 2011, pp. 1784-1790.
Magnusdottir et al., "Micropreparative capillary electrophoresis of DNA by direct transfer onto a membrane", Electrophoresis, vol. 18, 1997, pp. 1990-1993.
Martin et al., "Inkjet printing—the physics of manipulating liquid jets and drops", Engineering and Physics-Synergy for Success, IOP Publishing, Journal of Physics: Conference Series 105, 2008, pp. 1-14.
Morozov et al., "Electrospray Deposition as a Method for Mass Fabrication of Mono- and Multicomponent Microarrays of Biological and Biologically Active Substances", Anal. Chem., vol. 71, 1999, pp. 3110-3117.
Morozov et al., "Electrospray Deposition as a Method to Fabricate Functionally Active Protein Films", Anal. Chem, 1999, pp. 1415-1420.
PCT/US2017/045774, "International Preliminary Report on Patentability," dated Feb. 21, 2019, 9 pages.
PCT/US2017/045778, "International Preliminary Report on Patentability," dated Feb. 21, 2019, 9 pages.
Rejtar et al., "Off-Line Coupling of High-Resolution Capillary Electrophoresis to MALDI-TOF and TOF/TOF MS", Journal of Proteome Research, vol. 1(2), 2002, pp. 171-179.
Shi Jin et al., "Multiplexed Western Blotting Using Microchip Electrophoresis", Analytical Chemistry, vol. 88, No. 13, Jun. 2016, pp. 6703-6710.
Smith et al., "Sample Introduction and Separation in Capillary Electrophoresis, and Combination with Mass Spectrometric Detection," Talanta, vol. 36, No. 1/2, 1989, pp. 161-169.
Tracht et al., "Postcolumn Radionuclide Detection of Low-Energy β Emitters in Capillary Electrophoresis", Anal. Chem, 1994, pp. 2382-2389.
U.S. Appl. No. 14/791,023, "Notice of Allowance," dated Aug. 27, 2018, 11 pages.
U.S. Appl. No. 15/420,496, "Non-Final Office Action," dated Aug. 7, 2019, 11 pages.
U.S. Appl. No. 15/670,896, Advisory Action, dated Jul. 9, 2021, 3 pages.
U.S. Appl. No. 15/670,939, "Non-Final Office Action," dated Jul. 12, 2019, 15 pages.
Uematsu et al., "Surface morphology and biological activity of protein thin films produced by electrospray deposition", Journal of Colloid and Interface Science, vol. 269, 2004, pp. 336-340.
Wei et al., "Electrospray sample deposition for matrix-assisted laser desorption/ionization (MALDI) and atmospheric pressure MALDI mass spectrometry with attomole detection limits", Rapid Commun. Mass Spectrom, 2004, pp. 1193-1200.
Written Opinion for PCT/US2017/015657 dated Aug. 31, 2017, 14 pages.
Zhang et al., "Capillary Electrophoresis Combined with Matrix-Assisted Laser Desorption/Ionization Mass Spectrometry; Continuous Sample Deposition on a Matrix-precoated Membrane Target," Journal of Mass Spectrometry, Journal of Mass Spectrometry, , vol. 31, 1996, pp. 1039-1046.
Zhong et al., "Recent advances in coupling capillary electrophoresis-based separation techniques to ESI and MALDI-MS", Electrophoresis, vol. 35, 2014, pp. 1214-1225.

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US20180036729A1 (en)2018-02-08
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